Abstract

Human tuberculosis caused by Mycobacterium tuberculosis is the most prevalent and deadly bacterial infectious disease worldwide. This problem is compounded by the emergence of strains of M. tuberculosis that are resistant to one or more anti-tuberculous drugs. Following initial infections, M. tuberculosis frequently enters a latent or dormant state for extended periods and subsequently, under appropriate conditions or following immune suppression, revives, multiplies and causes a secondary infection. DNA replication constitutes an important step in the exit from latency. The development of novel therapeutic agents to control M. tuberculosis infections in HIV infected patients as well as other individuals is severely hindered by our limited understanding of the initiation and regulation of M. tuberculosis DNA replication and its coordination with other events in cell cycle. Initiation of DNA replication is believed to be triggered when DnaA, the putative initiator protein, interacts with oriC or origin of replication. Although oriC is essential for survival, some clinical strains of M. tuberculosis appear to tolerate major deletions and IS6110 insertions in their oriC, thereby raising questions as to how these clinical strains replicate their genome. Our research proposal focuses on understanding the replication initiation process in M. tuberculosis. Specifically, we propose to inactivate oriC, dnaA individually and together by homologous recombination in an attempt to determine whether replication in M. tuberculosis can proceed from alternate origins, and if so whether dnaA function is required for such replication. The interactions of DnaA with replication origins and consequences of these interactions will be investigated using biochemical and genetic approaches. To begin identifying the factors that could potentially affect DnaA activity, a proteomic approach combining two-dimensional gel electrophoretic separations of proteins with subsequent identification of protein spots by matrix-assisted laser ionization desorption/ionization mass spectrometry, will be used. Defining the molecular events involved in the initiation and regulation of replication is an essential prerequisite for developing defined systems for identifying novel antimycobacterial compounds, and thereby preventing the development of potentially lethal infections of M. tuberculosis.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
5R01AI041406-08
Application #
7013132
Study Section
Special Emphasis Panel (ZRG1-BM-1 (03))
Program Officer
Sizemore, Christine F
Project Start
1997-08-01
Project End
2008-01-31
Budget Start
2006-02-01
Budget End
2007-01-31
Support Year
8
Fiscal Year
2006
Total Cost
$194,996
Indirect Cost

  Institution

Name
University of Texas Health Center at Tyler
Department
Biochemistry
Type
Other Domestic Higher Education
DUNS #
800772337
City
Tyler
State
TX
Country
United States
Zip Code
75708

  Publications

Roberts, Gretta; Vadrevu, Indumathi S; Madiraju, Murty V et al. (2011) Control of CydB and GltA1 expression by the SenX3 RegX3 two component regulatory system of Mycobacterium tuberculosis. PLoS One 6:e21090
Madiraju, Murty; Madiraju, Sai Chandanda; Yamamoto, Kohji et al. (2011) Replacement of Mycobacterium smegmatis dnaA gene by Mycobacterium tuberculosis homolog results in temperature sensitivity. Tuberculosis (Edinb) 91 Suppl 1:S136-41
Maloney, Erin; Madiraju, Murty; Rajagopalan, Malini (2009) Overproduction and localization of Mycobacterium tuberculosis ParA and ParB proteins. Tuberculosis (Edinb) 89 Suppl 1:S65-9
Kiran, Manjot; Chauhan, Ashwini; Dziedzic, Renata et al. (2009) Mycobacterium tuberculosis ftsH expression in response to stress and viability. Tuberculosis (Edinb) 89 Suppl 1:S70-3
Maloney, Erin; Stankowska, Dorota; Zhang, Jian et al. (2009) The two-domain LysX protein of Mycobacterium tuberculosis is required for production of lysinylated phosphatidylglycerol and resistance to cationic antimicrobial peptides. PLoS Pathog 5:e1000534
Nair, Naveen; Dziedzic, Renata; Greendyke, Rebecca et al. (2009) Synchronous replication initiation in novel Mycobacterium tuberculosis dnaA cold-sensitive mutants. Mol Microbiol 71:291-304
Kiran, Manjot; Maloney, Erin; Lofton, Hava et al. (2009) Mycobacterium tuberculosis ftsZ expression and minimal promoter activity. Tuberculosis (Edinb) 89 Suppl 1:S60-4
Yamamoto, Kohji; Moomey, Meredith; Rajagopalan, Malini et al. (2008) Facilitation of dissociation reaction of nucleotides bound to Mycobacterium tuberculosis DnaA. J Biochem 143:759-64
Chauhan, Ashwini; Lofton, Hava; Maloney, Erin et al. (2006) Interference of Mycobacterium tuberculosis cell division by Rv2719c, a cell wall hydrolase. Mol Microbiol 62:132-47
Madiraju, Murty V V S; Moomey, Meredith; Neuenschwander, Pierre F et al. (2006) The intrinsic ATPase activity of Mycobacterium tuberculosis DnaA promotes rapid oligomerization of DnaA on oriC. Mol Microbiol 59:1876-90

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